Protective Effect of Transfection with Secretable Superoxide Dismutase (SOD) (a Signal Sequence-SOD Fusion Protein Coding cDNA) Expression Vector on Superoxide Anion-Induced Cytotoxicity in Vitro)
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概要
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For ex vivvo gene therapy, superoxide dismutase (SOD) must be secreted into the extracellular space and delivered to damaged cells. Recombinant DNA technique can be used to produce a secretory protein that is fused to a non-secretory protein and a signal peptide of another secretory protein gene. We constructed a secretable SOD eukaryotic expression vector which expressed human SOD cDNA by fusing it to the signal peptide DNA sequence of the human interleukin-2 (IL-2) gene. The ILSOD cDNA constructed by PCR-based gene expression was ligated into the multicloning site of the pRc/CMV plasmic (pRc/CMV-ILSOD). Rat lung epithelial like cells (L2 cells) were transfected with pRc/CMV-ILSOD by lipofection. The extracellular SOD activity of ILSOD-L2 cells (transfected cells with pRc/CMV-ILSOD) was 3 times as high as that of host cells.We used the xanthin (X)/ xanthin oxidase (XO) system to produce superoxide anions at the extracellular space. We initially investigated the direct cytotoxicity of superoxide anions upon cells. Host and ILSOD-L2 cells were killed by using X/XO, although the sensitivity of the ILSOD-L2 cells to X/XO induced cytotoxicity was significantly decreased compared with that of host cells. The production of lipid peroxidated substances in the host in the presence of X/XO increased to about twice the control (absence of X/XO) level. However, that of ILSOD-L2 cells did not change in the presence of X/XO. Therefore, ILSOD-L2 cells were resistant to X/XO induced lipid peroxidation. These findings indicated that ILSOD gene transfection protected against direct oxidant stress by X/XO.We then investigated the effect of extracellular SOD secreted from ILSOD-L2 cells on extracellular superoxide anion induced cytotoxicity in normal cells. The conditioned media of host cells had no significant effect upon X/XO induced cytotoxicity. However, the conditioned media of ILSOD-L2 cells protected against X/XO induced cytotoxicity. Furthermore, the conditioned medium of ILSOD-L2 cells was more effective than that of host cells against the production of lipid peroxidated substances by normal cells under conditions of oxidative stress. These results indicated that non-secretable protein could be delivered to target cells by means of DNA engineering. This strategy could thus provide an ex vivo means of applying gene therapy using non-secretable proteins.
- 公益社団法人日本薬学会の論文
- 1997-05-15
著者
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OKUMURA Katsuhiko
Department of Hospital Pharmacy, Kobe University School of Medicine
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Nishiguchi Kohshi
Department of Hospital Pharmacy, School of Medicine, Kobe University
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IWAKAWA Seigo
Kobe Pharmaceutical University
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Wu Xiao-ying
Department Of Pharmaceutics Faculty Of Pharmacy Kobe Pharmaceutical University
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Okumura K
Department Of Clinical Evaluation Of Pharmacotherapy Kobe University Graduate School Of Medicine
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IWAKAWA Seigo
Department of Pharmaceutics, Kobe Pharmaceutical University
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KOMADA Fusao
Department of Drug Informatics, Faculty of Pharmaceutical Sciences, Josai University
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Kamiyama Fumio
京都大学再生医科学研究所
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Kodama Fusao
Cosmed Pharmaceutical Co. Ltd.
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Iwakawa S
Department Of Cardiology Miki
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Iwakawa Seigo
Department Of Hospital Pharmacy School Of Medicine Kobe University : Department Of Pharmacy Kyoto Un
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Tanigawara Yusuke
Department Of Clinical Pharmacokinetics And Pharmacodynamics School Of Medicine Keio University
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Nishiguchi K
Department Of Hospital Pharmacy Kobe University School Of Medicine
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Nishiguchi Kohshi
Department Of Clinical Pharmacy Faculty Of Pharmaceutical Sciences Kyoto Pharmaceutical University
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Nishiguchi Kohshi
Department Of Hospital Pharmacy School Of Medicine Kobe University
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Ishida M
Shiseido Res. Center Kanagawa Jpn
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TANIGAWA Yasuke
Department of Hospital Pharmacy, School of Medicine, Kobe University
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ISHIDA Mariko
Department of Pharmaceutics, Faculty of Pharmacy, Kobe Pharmaceutical University
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SASADA Reiko
Biotechnology Laboratories, Central Research Division, Takeda Chemical Industries, Ltd.,
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Ishida Mariko
Department Of Pharmaceutics Faculty Of Pharmacy Kobe Pharmaceutical University
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Okumura Katsuhiko
Department Of Clinical Evaluation Of Pharmacotherapy Kobe University Graduate School Of Medicine
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Okumura Katsuhiko
Department Of Hospital Pharmacy Kyoto Pharmaceutical University:department Of Hospital Pharmacy Kobe
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Sasada R
Biotechnology Laboratories Central Research Division Takeda Chemical Industries Ltd.
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Komada F
Department Of Pharmacy Kobe University School Of Medicine
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Shinobu Ichikawa
Department Of Cardiology Miki
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Nakamura Takeshi
Department Of Gastroenterological Surgery Kobe University Graduate School Of Medical Sciences
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Nagahiro Kazumi
Department Of Hospital Pharmacy Kobe University School Of Medicine
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Ichikawa Shinobu
Department Of Cardiology Miki City Hospital
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Ishida Mariko
Department Of Human Nutrition School Of Life Studies Sugiyama Jogakuen University
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Iwakawa Seigo
Department of Cardiology, Miki
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